Process for efficient purification of neutral human milk oligosaccharides (HMOs) from microbial fermentation

ABSTRACT

The present application discloses a simple process for the purification of neutral human milk oligosaccharides (HMOs) produced by microbial fermentation. The process uses a combination of a cationic ion exchanger treatment, an anionic ion exchanger treatment, and a nanofiltration and/or electrodialysis step, which allows efficient purification of large quantities of neutral HMOs at high purity. Contrary to the purification currently used in fermentative production of neutral HMOs, the presented process allows the provision of HMOs without the need of a chromatographic separation. The so purified HMOs may be obtained in solid form by spray drying, as crystalline material or as sterile filtered concentrate. The provided HMOs are free of proteins and recombinant material originating from the used recombinant microbial strains and thus very well-suited for use in food, medical food and feed (e.g. pet food) applications.

CROSS-REFERENCE TO RELATED APPLICATIONS

This patent application is the U.S. national phase of International Application No. PCT/EP2014/079212, filed on Dec. 23, 2014, which claims the benefit of European Patent Application No. 14151737.5, filed Jan. 20, 2014, the disclosures of which are incorporated herein by reference in their entireties for all purposes.

The present application discloses a simple process for the purification of neutral human milk oligosaccharides (HMOs) produced by microbial fermentation. The process uses a combination of a cationic ion exchanger treatment, an anionic ion exchanger treatment, and a nanofiltration and/or electrodialysis step, which allows efficient purification of large quantities of neutral HMOs at high purity. Contrary to the purification currently used in fermentative production of neutral HMOs, the presented process allows the provision of HMOs without the need of a chromatographic separation. The so purified HMOs may be obtained in solid form by spray drying, as crystalline material or as sterile filtered concentrate. The provided HMOs are free of proteins and recombinant material originating from the used recombinant microbial strains and thus very well-suited for use in food, medical food and feed (e.g. pet food) applications.

Human milk represents a complex mixture of carbohydrates, fats, proteins, vitamins, minerals and trace elements. The by far most predominant fraction is represented by carbohydrates, which can be further divided into lactose and more complex oligosaccharides. Whereas lactose is used as an energy source, the complex oligosaccharides are not metabolized by the infant. The fraction of complex oligosaccharides accounts for up to 1/10 of the total carbohydrate fraction and consists of probably more than 150 different oligosaccharides. The occurrence and concentration of these complex oligosaccharides are specific to humans and thus cannot be found in large quantities in the milk of other mammals, like for example domesticated dairy animals.

The existence of these complex oligosaccharides in human milk is known already for a long time and the physiological functions of these oligosaccharides were subject to medicinal research for many decades (Gura, T. (2014) Nature's first functional food. Science 345(6198) 747-749). For some of the more abundant human milk oligosaccharides, specific functions have already been identified (Bode, L. (2012) Human milk oligosaccharides: every baby needs a sugar mama. Glycobiology 22(9), 1147-1162.; Bode L, Jantscher-Krenn E (2012) Structure-function relationships of human milk oligosaccharides. Adv Nutr 3(3) 383S-391S; Morrow A L, Ruiz-Palacios G M, Altaye M, Jiang X, Guerrero M L, Meinzen-Derr J K, Farkas T, Chaturvedi P, Pickering L K, Newburg D S (2004) Human milk oligosaccharides are associated with protection against diarrhea in breast-fed infants. J Pediatr 145(3) 297-303).

The limited supply and difficulties of obtaining pure fractions of individual human milk oligosaccharides lead to the development of chemical routes to some of these complex molecules. However, synthesis of human milk oligosaccharides by chemical synthesis, enzymatic synthesis or fermentation proofed to be challenging. At least large-scale quantities as well as qualities sufficient for food applications cannot be provided until today. In this regard, particularly chemical synthetic routes to human milk oligosaccharides (e.g. 2′-fucosyllactose; see WO 2010/115935 A1) involve several noxious chemicals, which impose the risk to contaminate the final product.

Due to the challenges involved in the chemical synthesis of human milk oligosaccharides, several enzymatic methods and fermentative approaches were developed (Miyazaki et al., (2010) Methods in Enzymol. 480, 511-524; Murata et al., (1999) Glycoconj. J. 16, 189-195; Baumgartner, F. et al., (2013) Microb. Cell Fact. 12, 40; Lee et al., (2012) Microb. Cell Fact. 11, 48; U.S. Pat. No. 7,521,212 B1 or Albermann et al., (2001) Carbohydr. Res. 334(2) p 97-103). However, these methods—yield complex mixtures of oligosaccharides i.e. the desired product is contaminated with starting material such as lactose, biosynthetic intermediates and substrates such as individual monosaccharides and polypeptides etc.

Processes in the state of the art for purifying individual oligosaccharide products from these complex mixtures are technically complex and also uneconomical for food applications. For the purification of the disaccharides lactose or sucrose from complex mixtures such as whey or molasses, industrial scale processes have been developed which involve multiple crystallizations. The disadvantage of said methods is that they are elaborate and only lead to low yields.

For the purification of complex oligosaccharides from microbial fermentation, such as certain human milk oligosaccharides, gel-filtration chromatography is the method of choice until now. The disadvantage of gel-filtration chromatography is that it cannot be efficiently scaled up and it is unsuitable for continuous operation. Thus, gel-filtration chromatography is not economical and renders it impossible to provide certain human milk oligosaccharides—like 2′-fucosyllactose or lacto-N-tetraose—in reasonably amounts and quality to use them in human food or other applications such as animal food (e.g. pet food). The application as animal feed or pet food is interesting on the basis that also other mammals contain the same or similar neutral complex oligosaccharides in their milk as humans (e.g. 2′-fucosyllactose is also found in the milk of dogs, pigs, chimpanzee) (Castanys-Munzo, E., Martin, J. M & Prieto, P. A. (2013) 2′-fucosyllactose: an abundant, genetically determined soluble glycan present in human milk. Nutr. Rev. 71(12) 773-789).

Another problem is presented by the use of recombinant strains (recombinant bacterial or yeast strains) in the microbial fermentation, resulting in the contamination of the fermentation product with recombinant material. However, contamination with recombinant DNA or proteins is not acceptable by regulators and consumers today. Detection limits in particular for recombinant DNA molecules are very low. In case qPCR based detection is used, which is currently regarded as the gold standard for detection, even as little a single DNA molecules can be detected. Proteins in addition pose the risk of allergic reactions and should therefore be efficiently removed from the desired oligosaccharide product.

Electrodialysis (ED) represents a technique combining dialysis and electrolysis and can be used for the separation or concentration of ions in solutions based on their selective electromigration through semipermeable membranes. First industrial applications of electrodialysis dated back into the early 1960 with the demineralization of cheese whey for the use in infant formula. Further developed applications of electrodialysis include the adjustment of pH of beverages such as wines, grape must, apple juice and orange juice.

The desalination for brackish water for the production of drinking water and the demineralization of milk whey for infant food production represent the largest area of application, today.

The basic electrodialysis principle consists of an electrolytic cell composed of a pair of electrodes submerged into an electrolyte for conduction of ions connected to a direct current generator. The electrode connected to the positive pole of the direct current generator is the anode, and the electrode connected to the negative pole is called cathode. The electrolyte solution then supports the current flow, which results from the movement of negative and positive charge ions towards the anode and cathode respectively. The membranes employed in the electrodialysis are essentially sheets of porous ion-exchange resins, owing negative or positive charge groups and therefore addressed as cationic or anionic membrane, respectively. The ion exchanger membranes are usually made of polystyrene carrying a suitable functional group (such as sulfonic acid or a quaternary ammonium group for cationic or anionic membranes, respectively) cross-linked with divinylbenzene. As electrolyte, sodium chloride, or sodium acetate, sodium propionate etc. can be employed. The electodialysis stack is then assembled in such a way that the anionic and cationic membranes are parallel as in a filter press between two electrode blocks that the stream undergoing ion depletion is well separated from the stream undergoing ion enrichment (the two solutions are also referred to as diluate (undergoing ion depletion) and concentrate (undergoing ion enrichment). The heart of electrodialysis process is the membrane stack, which consists of several anion and cation-exchange membranes separated by spacers, and installed between two electrodes. By applying a direct electric current, anions and cations will migrate across the membranes towards the electrodes generating a diluate (desalted) and a concentrate stream.

Generally, the pore size of the employed membranes is rather small in order to prevent diffusion of the product from the diluate into the concentrate stream, driven by the often high concentration differences between the two streams. After separation from biomass, proteins and in particular recombinant DNA molecules (in the size of entire genomes) have to be removed quantitatively from the desired product. If at all possible the electrodialysis of such large molecules (in comparison to the molecular size of HMOs) would be rather lengthy and surely accompanied with significant losses of the desired product from the diluate into the concentrate.

Diafiltration is a process that involves the addition of fresh water to a solution in order to “wash out” or remove membrane permeable components. Thus, diafiltration can be used to separate components on the basis of their molecular size by using appropriate membranes, wherein one or more species are efficiently retained and other species are membrane permeable. In particular, diafiltration by using a nanofiltration membrane is effective for the separation of low molecular compounds from salts. In general, nanofiltration membranes possess a molecular weight cut-off in the range of 150 to 300 Daltons. Today, nanofiltration (NF) is widely used in the dairy industry for the concentration and demineralization of whey. Nanofiltration has already been employed for the enrichment of a human milk oligosaccharide fraction form human milk. In this approach, nanofiltration has been used in combination with enzymatic degradation of lactose to separate the HMO fraction from the milk lactose (Sarney D. B, Hale, C., Frankel, G & Vulfson, E. N. (2000) A novel approach to the recovery of biological active oligosaccharides from milk using a combination of enzymatic treatment and nanofiltration. Biotechnol. Bioeng 69, 461-467.

In the developed process for the efficient purification of food-grade human milk oligosaccharides from microbial fermentation, nanofiltration is employed in order to concentrate the desired product and also to remove membrane permeable salts.

Starting from this prior art, the technical problem is the provision of a novel process to provide neutral HMOs in high amounts, high purity and excellent yields.

The technical problem is solved by the process according to claim 1, the human milk oligosaccharide (HMO) according to claim 15 and the use of the HMO according to claim 19. The dependent claims display advantageous embodiments.

The present invention provides a process for purification of neutral human milk oligosaccharides (HMO) in a batch manner or in a continuous manner from a fermentation broth obtained by microbial fermentation wherein a purified solution comprising a neutral HMO at a purity of ≥80% is provided. The fermentation broth contains the neutral HMO, biomass, medium components and contaminants. The purity of the neutral HMO in the fermentation broth is <80%.

During the process the fermentation broth is applied to the following purification steps:

i) Separation of biomass from the fermentation broth,

ii) Cationic ion exchanger treatment for the removal of positively charged material,

iii) Anionic ion exchanger treatment for the removal of negatively charged material,

iv) Nanofiltration step (comprising or consisting of concentration and/or diafiltration of the neutral HMO) and/or electrodialysis step (especially for the removal of salts and other low molecular weight compounds).

Contaminants present in the cell-free fermentation broth are for example other oligosaccharides than the desired neutral HMO, like monovalent and divalent salts, amino acids, polypeptides, proteins, organic acids, nucleic acids, etc. The desired neutral HMO can be obtained at a purity of ≥80% in the purified solution.

The applicant has discovered that with the inventive purification process, an efficient purification of neutral HMOs from microbial fermentation can be attained, which delivers the HMO at purity suitable for food and feed applications. Furthermore the process is highly cost effective because no chromatographic separation step is needed. Furthermore, it has been discovered that the purity of ≥80% is achieved whether an electrodialysis step or a nanofiltration step is performed in step iv) or if both steps are performed in succession.

One advantage of the process according to the present is that the desired neutral HMOs are obtained free from DNA and proteins from the used recombinant microbial fermentation strain. Especially the implementation of a cationic ion exchanger treatment (step ii) allows the removal of positively charged material like e.g. positively charged proteins. Consequently, the inventive method provides an HMO which comprises less positively charged contaminant material compared to conventional purification schemes known in the prior art which do not implement a cationic exchanger treatment. It was further discovered that after passing the fermentation broth separated from the biomass (preferably by ultrafiltration) over a cationic ion exchanger (in proton form), the obtained solution was stable and could be stored at room temperature or under cooling for several weeks. Furthermore, the obtained neutral HMO is free of recombinant material, as judged by quantitative PCR with up to 50 amplification cycles. Moreover, the product obtained from the process according to the invention is characterized by low amounts or absence of proteins.

Furthermore, the neutral HMO purification according to the invention is highly efficient with yet unknown yields of >70% (optionally >75%) of the purified HMO (determined from cell free fermentation medium to HMO concentrate).

Thus, a hybrid process is provided comprising the steps of separation of biomass, ion exchanger, and a step of nanofiltration and/or electrodialysis, and preferably further comprising an activated carbon treatment, for the efficient provision of neutral HMOs at high purity free of recombinant genetic material, endotoxins and proteins form fermentation processes using recombinant fermentation strains. With the process according to the invention, large amounts of high quality human milk oligosaccharides may be provided in a very convenient and economical way.

The neutral HMO may be purified from a fermentation broth obtained by microbial fermentation using a recombinant microorganism, preferably bacteria or yeast, more preferably a recombinant microorganism grown in a chemically defined medium. Optionally, the biomass separated in step i) is recycled to the microbial fermentation.

In another preferred embodiment of the process according to the invention, the purity of the neutral HMO in the fermentation broth is ≤70%, ≤60%, ≤50%, ≤40%, ≤30%, ≤20%, ≤10% or ≤5% and/or the purified solution contains the neutral HMO at a purity of ≥85%, preferably of ≥90%.

In another preferred embodiment of the process according to the invention, the yield of the neutral HMO is >70% (optionally >75%) and/or the purified solution is free of DNA, proteins, and/or recombinant genetic material.

In another preferred embodiment of the process according to the invention, the neutral HMO is selected from the group consisting of 2′-fucosyllactose, 3-fucosyllactose, 2′,3-difucosyllactose, lacto-N-triose II, lacto-N-tetraose, lacto-N-neotetraose, lacto-N-fucopentaose I, lacto-N-neofucopentaose, lacto-N-fucopentaose II, lacto-N-fucopentaose III, lacto-N-fucopentaose V, lacto-N-neofucopentaose V, lacto-N-difucohexaose I, lacto-N-difucohexaose II, 6′-galactosyllactose, 3′-galactosyllactose, lacto-N-hexaose and lacto-N-neohexaose.

In a particularly preferred embodiment of the process according to the invention, the neutral HMO is 2′-fucosyllactose.

In another preferred embodiment of the process according to the invention, the separation of biomass from the fermentation broth is achieved by

a) ultrafiltration, preferably by separating biomass and materials >500 kDa, more preferably >150 kDa; and/or

b) filtration through a cross-flow filter, preferably with a cut-off ≤100 kDa, more preferably with a cut-off ≤10 kDa, even more preferably a cut-off ≤5 kDa;

wherein step a) is preferably implemented before step b).

In another preferred embodiment of the process according to the invention, at least one of the purification steps ii) to v) of the inventive process is repeated at least one time during the process.

In another preferred embodiment of the process according to the invention, the fermentation broth is applied at least one time to an activated carbon treatment after at least one of the purification steps i) to iv) for the adsorption of colour giving material and larger oligosaccharides to activated carbon. By applying the fermentation broth to this additional purification step, colour giving material and larger oligosaccharides can be removed from the fermentation broth.

The inventive process may be characterized in that

a) after at least one of the purification steps i) to iv); or

b) after at least one activated carbon treatment for the adsorption of colour giving material and larger oligosaccharides to activated carbon; or

c) before a concentration step which is implemented after at least one of the purification steps i) to iv);

the solution comprising the neutral human milk oligosaccharide is diafiltered and/or concentrated. Preferably, said solution is diafiltered and/or concentrated with a nanofiltration membrane, more preferably with a nanofiltration membrane having a size exclusion limit of ≤20 Å. Most preferably, the solution is diafiltered until a conductivity of ≤15 mS/cm, preferably ≤10 mS/cm, more preferably ≤5 mS/cm, is reached.

Diafiltration using nanofiltration was found efficient as a pretreatment to remove significant amounts of contaminants prior to an electodialysis treatment of the HMO containing solution. In addition, nanofiltration was also found to be efficient in the removal of low molecular contaminants after an ultrafiltration step, wherein said removal is beneficial for concentrating and demineralizing the HMO solution prior to ion-exchanger treatment. The use of nanofiltration membranes for concentration and diafiltration in the purification of human milk oligosaccharides results in lower energy and processing cost, as well as in improved product quality, due to reduced thermal exposure, leading to reduced Maillard reactions and aldol reactions.

In a step before step i), a glucosidase treatment, preferably a β-glucosidase treatment, may be performed with the fermentation broth, wherein said treatment is preferably performed by

a) adding a microorganism strain capable of expressing one or more glycosidase enzyme(s) which are suitable for the degradation of unwanted intermediates, substrates and/or oligosaccharide side products; and/or

b) using a fermentation strain that expresses one or more glycosidase enzymes(s), preferably by adding an inducer to the fermentation broth and/or by shifting the temperature of the fermentation broth; and/or

c) adding one or more glycosidase(s), preferably at least a β-glucosidase, to the fermentation broth as a crude enzyme or as a purified enzyme.

In another preferred embodiment of the process according to the invention, the fermentation broth is concentrated after at least one of the purification steps i) to iv), preferably after purification step iv), using vacuum evaporation or reverse osmosis or nanofiltration (e.g. nanofiltration with a nanofiltration membrane having a size exclusion limit of ≤20 Å)

a) to a concentration of ≥100 g/L, preferably ≥200 g/L, more preferably ≥300 g/L; and/or

b) at a temperature of <80° C., preferably <50° C., more preferably 20° C. to 50° C., even more preferably 30° C. to 45° C., most preferably 35° C. to 45° C. (specifically relevant for vacuum evaporation or reverse osmosis); and/or

c) at a temperature of <80° C., preferably <50° C., more preferably 4° C. to 40° C. (specifically relevant for nanofiltration).

In another preferred embodiment of the process according to the invention, the purified solution is sterile filtered and/or subjected to endotoxin removal, preferably by filtration of the purified solution through a 3 kDa filter.

In another preferred embodiment of the process according to the invention, the neutral HMO containing solution is subjected to electrodialysis in order to further remove charged materials such as mono- and divalent salts.

In another preferred embodiment of the process according to the invention, the purified solution is concentrated to a concentration of >1.5 M and cooled to a temperature <25°, more preferable <8° C., to obtain crystalline material of the neutral HMO.

In another preferred embodiment of the process according to the invention, the purified solution is spray-dried, particularly spray-dried at a concentration of the neutral HMO of 20-60 (w/v), preferably 30-50 (w/v), more preferably 35-45 (w/v), a nozzle temperature of 110-150° C., preferably 120-140° C., more preferably 125-135° C. and/or an outlet temperature of 60-80° C., preferably 65-70° C.

Furthermore, the present invention includes a neutral human milk oligosaccharide (HMO) that is producible with the process according to the invention.

In a preferred embodiment, the HMO is present in a sterile filtered concentrate, e.g. sterile concentrate containing neutral HMO product with a concentration of ≥30% (w/v), more preferably ≥40% (w/v).

In another preferred embodiment, the HMO is spray-dried or crystallized.

In another preferred embodiment, the HMO is selected from the group consisting of 2′-fucosyllactose, 3-fucosyllactose, 2′,3-difucosyllactose, lacto-N-triose II, lacto-N-tetraose, lacto-N-neotetraose, lacto-N-fucopentaose I, lacto-N-neofucopentaose, lacto-N-fucopentaose II, lacto-N-fucopentaose III, lacto-N-fucopentaose V, lacto-N-neofucopentaose V, lacto-N-difucohexaose I, lacto-N-difucohexaose II, 6′-galactosyllactose, 3′-galactosyllactose, lacto-N-hexaose and lacto-N-neohexaose.

In a particularly preferred embodiment, the HMO is 2′-fucosyllactose.

In another preferred embodiment, the HMO has

a) a conductivity of less than 1 mSi/cm at a 300 g/l solution;

b) is free of recombinant DNA material, optionally free of any DNA; and/or

c) is free of proteins derived from the recombinant microorganism, optionally free of any proteins.

Another preferred embodiment is directed to an HMO for use in medicine, preferably for use in prophylaxis or therapy of a gastrointestinal disorder.

Furthermore, the present invention includes the use of an HMO according to the invention as additive in food, preferably as additive in human food and/or pet food, more preferably as additive in human baby food.

The subject according to the application is intended to be explained in more detail with reference to the subsequent figures and examples without wishing to restrict said subject to the special embodiments.

FIG. 1 shows a scheme of a preferred embodiment of the process according to the present invention for the purification of 2′-fucosyllactose from a fermentation broth comprising the steps: ultrafiltration, cationic and anionic ion exchanger treatment, activated carbon treatment, nanofiltration, electrodialysis and concentration.

FIG. 2 shows a scheme of another preferred embodiment of the process according to the present invention for the purification of 2′-fucosyllactose from a fermentation broth comprising the steps: ultrafiltration, nanofiltration, cationic and anionic ion exchanger treatment, activated carbon treatment, electrodialysis and concentration.

FIG. 3 shows a scheme of another preferred embodiment of the process according to the present invention for the purification of 2′-fucosyllactose from a fermentation broth comprising the steps: ultrafiltration, cationic and anionic ion exchanger treatment, nanofiltration, activated carbon treatment, electrodialysis and concentration.

EXAMPLE 1: PURIFICATION OF 2′-FUCOSYLLACTOSE FROM FERMENTATION USING A RECOMBINANT MICROBIAL PRODUCTION STRAIN I

A 2′-fucosyllactose feed-batch fermentation employing a recombinant 2′-fucosyllactose synthesizing E. coli strain (E. coli BL21(DE3) ΔlacZ), containing a genomic integration 2′-fuosyltranferase, encoded by the wbgL gene (see EP 11 1151 571.4), and having an additional copy of the E. coli lacY, manB, manC, gmd and fcl all under the control of a strong constitutive tetracyclin promoter, containing a functional gal operon comprising the genes galM, galK, galT and galE, was grown in a defined salt medium. The defined salt medium comprised 7 g l⁻¹ NH₄H₃PO₄, 7 g l⁻¹ K₂HPO₄, 2 g l⁻¹ KOH, 0.37 g l⁻¹ citric acid, 1 mll⁻¹ antifoam (Struktol J673, Schill+Seilacher), 1 mM CaCl₂, 4 mM MgSO₄, trace-elements and 2% glycerol as carbon source.

Trace elements consisted of 0.101 g l⁻¹ nitrilotriacetic acid, pH 6.5, 0.056 g l⁻¹ ammonium ferric citrate, 0.01 g l⁻¹ MnCl₂×4H₂O, 0.002 g l⁻¹ CoCl₂×6H₂O, 0.001 g l⁻¹ CuCl₂×2H₂O, 0.002 g l⁻¹ boric acid, 0.009 g l⁻¹ ZnSO₄×7H₂O, 0.001 g l⁻¹ Na₂MoO₄×2H₂O, 0.002 g l⁻¹ Na₂SeO₃, 0.002 g l⁻¹ NiSO₄×6H₂O.

Glycerol-feed consisted of glycerol 800 g l⁻¹, MgSO₄ 2.64 g l⁻¹ and trace element solution 4 mll⁻¹. For 2′-fucosyllactose formation, a lactose feed of 216 g l⁻¹ was employed. The pH was controlled by using ammonia solution (25% v/v). Feed batch fermentation was cultured at 30° C. under constant aeration and agitation for 90 hours. At 90 hours after the start of the fermentation, most of the added lactose was converted into 2′-fucosyllactose. In order to remove lactose still present in the fermentation supernatant, a second bacterial strain was added to the fermentation vessel 90 hours after the fermentation start.

The added second bacterial strain was genetically identical to the first employed bacteria strain, differing, however, only in the expression of a genome integrated beta-galactosidase. Incubation of the added secondary bacterial strain resulted in the disappearance of the residual lactose within 5 hours. Approximately 10 ml starter culture of the second beta-galactosidase expressing bacterial strain was added per 1 l fermentation broth.

The biomass was then separated from the fermentation medium by ultrafiltration, using a cross-flow filter with a cut-off of 10 kDa (Microdyn Nardir).

An approximately 1 m³ cell-free fermentation medium was obtained containing 42 g/l 2′-fucosyllactose. The cell-free fermentation medium was then passed over a strong cationic ion exchanger (Lewatit S 6368 A (Lanxess) in H⁺ form, size of ion exchanger bed volume was 100 l), in order to remove positive charged contaminants. The obtained solution was then set to pH 7 by the addition of a 2 M sodium hydroxide solution.

The solution was then (without delay) passed over an anionic ion exchanger column (bed volume of ion exachanger was 100 l). The used strong anionic ion exchanger Lewatit S 2568 (Lanxess) was in chloride (Cl⁻) form. The obtained solution was again neutralized to pH 7. The thus obtained solution was then diafiltrated using an Alfa-Laval NF99HF nanofiltration membrane and six volumes of sterile deionized water. The solution was further concentrated using the nanofiltration membrane wherein a 2′-fucosyllactose solution of 200 g/l and a conductivity of 7 mS/cm was obtained.

The concentrated 2′-fucosyllactose solution was then treated with activated carbon in order to remove color giving material such as Maillard reaction products and aldol reaction products. As activated carbon 20 g Norit GAC EN per I concentrated 2′-fucosyllactose solution was used, yielding a significantly decolorized solution.

The thus obtained concentrated 2′-fucosyllactose solution was then electrodialysed to 0.3 mS/cm using a PC-Cell BED 1-3 electrodialysis apparatus (PC-Cell, Heusweiler, Germany) equipped with PC-Cell E200 membrane stack. Said stack contained the following membranes: cation exchange membrane CEM: PC SK and the anion exchange membrane AEM:PcAcid60 having a size exclusion limit of 60 Da. A 0.025 M sulfamic acid (amidosulfonic acid) solution was used as an electrolyte in the ED process.

Then, the obtained solution was then concentrated under vacuum at 40° C. to obtain a 45% 2′-fucosyllactose solution. The concentrated solution was then again treated with ion exchangers, Lewatit S 6368 A (Lanxess) in Na⁺ form (bed volume of the used ion exchanger was 10 l) and after neutralization with the anionic ion exchanger Lewatit S 2568 (Lanxess) in Cl⁻ form (bed volume of the employed ion exchanger was 10 l).

The obtained 2′-fucosyllactose solution was then treated with activated carbon (Norit DX1 Ultra). For 1 l of a 45% 2′-fucosyllactose solution 30 g activated carbon were employed.

The solution was then again subjected to electrodialysis until a conductivity of less than 0.3 mSi/cm was obtained.

Subsequently, the solution was subjected to sterile filtration by passing the solution through a 3 kDa filter (Pall Microza ultrafiltration hollow fiber module SEP-2013, Pall Corporation, Dreieich).

Part of the obtained 2′-fucosyllactose solution was then spray dried for analysis.

For NMR spectra recording the spray-dried product was dissolved in hexadeuterodimethyl sulfoxide (DMSO-d₆). For the proton and ¹³C analysis the following characteristic chemical shifts were observed:

¹H NMR (500 MHz, DMSO-d₆) δ6.63 (d, J=6.5 Hz, 1H), 6.28 (d, J=4.7 Hz, 1H), 5.21 (d, J=2.4 Hz, 1H), 5.19 (d, J=2.4 Hz, 1H), 5.01 (d, J=2.2, 2H), 4.92 (d, J=5.0 Hz, 1H), 4.89 (dd, J=4.6, 1.3 Hz, 2H), 4.78 (d, J=5.3 Hz, 1H), 4.74 (d, J=5.1 Hz, 1H), 4.63 (m, 6H), 4.53 (t, d, J=5.5, 1H), 4.46 (d, J=5.2 Hz, 1H), 4.44 (d, J=5.0 Hz, 1H), 4.38-4.26 (m, 5H), 4.23 (d, J=0.9, 1H), 4.05 (d, J=0.9, 1H), 4.00 (quin, J=3.3, 1H), 3.68-3.60 (m, 7H), 3.59-3.50 (m, 13H), 3.50-3.37 (m, 6H), 3.24 (dt, J=8.8, 2.2 Hz, 1H), 3.14 (m, 2H), 2.96 (td, J=8.4, 4.7 Hz, 1H), 1.04 (d, J=6.1 Hz, 3H), 1.03 (d, J=6.1 Hz, 3H).

¹³C NMR (126 MHz, DMSO-d₆) δ100.99, 100.85, 100.35, 100.25, 96.59, 92.02, 78.13, 77.78, 77.16, 77.01, 75.27 75.05, 74.67, 73.70, 72.33, 71.62, 71.56, 70.91, 69.90, 69.64, 68.75, 68.16, 66.33, 60.17, 59.82, 59.67, 16.37, 16.36.

Chemicals shifts were found to be consistent with the 2′-fucosyllactose structure.

Using this protocol a 45% 2′-fucosyllactose concentrate with a purity of 94.5% could be obtained (determined by HPLC analysis). Major contaminants were 3′-fucosyllactose (1.8%), difucosyllactose (2.9%), and lactose (0.3%).

The yield of the purification was approximately 70%.

Importantly, no recombinant material could be determined in 10 g of freeze material using 50 cycles of qPCR. Protein amount of the obtained material was determined as <50 peg freeze dried material by using a nano-Bradford assay (Roth, Karlsruhe Germany). Total amount of ash was determined with 0.19%.

Concentration of heavy metals was (arsenic cadmium, lead and mercury) below 0.1 μg/g material. Endotoxin levels were determined to be <0.005 EU/ml 2′-fucosyllactose concentrate.

EXAMPLE 2: PURIFICATION OF 2′-FUCOSYLLACTOSE FROM FERMENTATION USING A RECOMBINANT MICROBIAL PRODUCTION STRAIN II

A 1 m³ microbial fermentation comprising 2′-fucosyllactose at a concentration of 47 g/L was filtered through a cross flow filter with a cut off of 100 kDa (Microdyn Nadir) to obtain a cell free fermentation medium.

As a fermentation medium the following medium was employed: Major medium components: glycerol 30 g/l, NH₄H₂PO₄ 7 g/l, K₂HPO₄ 7 g/l, citrate 0.3 g/l, KOH 2 g/l, MgSO₄.7H₂O 2 g/l; trace elements: CaCl₂.6H₂O 20 mg/l, nitrilotriacetic acid 101 mg/l, ammonium ferric citrate 56 mg/l, MnCl₂.4H₂O 9.8 mg/l, CoCl₂.6H₂O 1.6 mg/l, CuCl₂.2H₂O 1 mg/l, H₃BO₃1.6 mg/l, ZnSO₄.7H₂O 9 mg/l, Na₂MoO₄.2H₂O 1.2 mg/l, Na₂SeO₃ 1.2 mg/l; feed substances: glycerol and lactose.

The cell free fermentation medium was then passed over a cationic ion exchanger (Lewatit S 6368 A (Lanxess) in H⁺ form (volume of ion exchanger bed was 100 l) in order to remove positive charged contaminants. The obtained solution was then set to pH 7 by the addition of a 2 M sodium hydroxide solution. The solution was then, without delay passed over an anionic ion exchanger column (ion exchanger bed volume used was 100 l) comprising the strong anionic ion exchanger Lewatit S 2568 (Lanxess) in chloride (Cl⁻) form. The obtained solution was again neutralized to pH 7. The so obtained solution was then diafitrated (using 10 volumes of sterile deionized water) and concentrated using a nanofiltration membrane (Alfa-Laval NF99HF) to obtain a 2′-fucosyllactose solution of 200 g/l and a conductivity of approx. 7 mSi/cm.

The concentrated 2′-fucosyllactose solution was then treated with activated carbon, using 20 g Norit GAC EN per I concentrated 2′-fucosyllactose solution. To the filtered 2′-fucosyllactose solution 40 g/l Norit DX1 Ultra activated carbon was added. The solution was then exposed to the activated carbon at 4° C. for approximately 18 h. After 18 h, the activated carbon was removed from the 2′-fucosyllactose solution by filtration.

The solution was then electrodialysed to a conductivity of <0.3 mS/cm using a PC-Cell BED 1-3 electrodialysis apparatus (PC-Cell, Heusweiler, Germany) equipped with PC-Cell E200 membrane stack. Said stack contained the following membranes: cation exchange membrane CEM: PC SK and the anion exchange membrane AEM:PcAcid60 having a size exclusion limit of 60 Da. A 0.025 M sulfamic acid (amidosulfonic acid) solution was used as an electrolyte in the ED process.

The obtained solution was then concentrated to obtain a 40% 2′-fucosyllactose solution. The obtained 2′-fucosyllactose solution was then passed over a Lewatit S 2568 (Lanxess) Cl⁻ form (bed volume 101) and treated with activated carbon (Norit DX1 Ultra) at 8° C. for 18 h. The solution was then subjected to sterile filtration by passing the solution through a 3 kDa filter

(Pall Microza ultrafiltration hollow fiber module SEP-2013, Pall Corporation, Dreieich) and spray-dried using a NUBILOSA LTC-GMP spray dryer (NUBILOSA, Konstanz, Germany).

Using this protocol, 2′-fucosyllactose with a purity of 94% could be obtained (determined by HPLC analysis). Major contaminants were 3′-fucosyllactose (1.8%), difucosyllactose (3.2%) and lactose (0.2%). The yield of the purification was approximately 70%. 

The invention claimed is:
 1. A process for the purification of 2′-fucosyllactose in a batch manner or in a continuous manner from a fermentation broth obtained by microbial fermentation, wherein the fermentation broth comprises kilogram amounts of 2′-fucosyllactose, which process comprises i) separating the microbial biomass from the fermentation broth; ii) subjecting the separated fermentation broth obtained in step i) to a cation exchanger or to an anion exchanger to obtain a solution; iii) subjecting the solution obtained in step ii) to the cation or anion exchanger not used in step ii); iv) subjecting the solution obtained from step iii) to nanofiltration or reverse osmosis or vacuum evaporation to obtain a purified solution of 2′-fucosyllactose; v) optionally treating the purified solution obtained from step iv) with activated carbon; wherein the 2′-fucosyllactose in the purified solution obtained after step iv) or step v) has a purity of ≥80% as determined by HPLC.
 2. The process of claim 1, wherein the separating step i) is performed using ultrafiltration using a cross-flow filter.
 3. The process of claim 1, wherein the solution obtained after step iii) is diafiltrated before step iv).
 4. The process of claim 1, wherein after step iv), the 2′-fucosyllactose is concentrated to between about 100 g/L to 300 g/L.
 5. The process of claim 1, wherein step iv) is performed using nanofiltration.
 6. The process of claim 1, wherein the optional activated carbon treatment step v) is performed.
 7. The process of claim 6, further comprising subjecting the purified solution to electrodialysis before or after step v).
 8. The process of claim 7, wherein the electrodialysis comprises use of cation and/or anion exchangers.
 9. The process of claim 1, wherein the pH is adjusted to about 7 after step ii) and after step iii).
 10. The process of claim 1, further comprising concentrating the purified solution obtained after step iv) or optional step v).
 11. The process of claim 1, further comprising spray drying the purified solution from step iv) or optional step v) to obtain a purified, solid form of 2′-fucosyllactose.
 12. The process of claim 7, further comprising concentrating the solution after the electrodialysis.
 13. The process of claim 6, comprising further subjecting the purified solution from step v) to a cation and/or anion exchanger to obtain a further purified solution.
 14. The process of claim 13 further comprising treating the further purified solution with activated carbon.
 15. The process of claim 14, further comprising subjecting the further purified solution to nanofiltration, electrodialysis and/or reverse osmosis.
 16. The process of claim 15, further comprising spray drying the solution to obtain a purified, solid form of 2′-fucosyllactose.
 17. The process of claim 1, further comprising adding a β-glucosidase to the fermentation broth prior to step i).
 18. A process for the purification of 2′-fucosyllactose in a batch manner or in a continuous manner from a fermentation broth obtained by microbial fermentation, wherein the fermentation broth comprises kilogram amounts of 2′-fucosyllactose, which process comprises i) separating the microbial biomass from the fermentation broth; ii) subjecting the separated fermentation broth obtained in step i) to nanofiltration; iii) subjecting the separated fermentation broth obtained in step ii) to a cation exchanger or to an anion exchanger to obtain a solution; iv) subjecting the solution obtained in step iii) to the cation or anion exchanger not used in step iii) to obtain a purified solution; v) optionally treating the purified solution obtained from step iv) with activated carbon; wherein the 2′-fucosyllactose in the purified solution obtained after step iv) or optional step v) has a purity of ≥80% as determined by HPLC.
 19. The process of claim 18, wherein the separating step i) is performed using ultrafiltration using a cross-flow filter.
 20. The process of claim 18, wherein the separated fermentation broth obtained in step i) is diafiltrated before step ii).
 21. The process of claim 18 wherein after step ii), the 2′-fucosyllactose is concentrated to between about 100 g/L to about 300 g/L.
 22. The process of claim 18, wherein the activated carbon treatment step v) is performed.
 23. The process of claim 22, further comprising subjecting the solution to electrodialysis before or after step v).
 24. The process of claim 23, further comprising concentrating the purified solution by vacuum evaporation or reverse osmosis.
 25. The process of claim 24, further comprising spray drying the purified solution to obtain a purified, solid form of 2′-fucosyllactose.
 26. The process of claim 18, further comprising adding a β-glucosidase to the fermentation broth prior to step i). 